Test 3 CRISPR/Cas Flashcards
Describe how the CRISPR/Cas system works in bacteria?
- Foreign DNA acquisition
- Viral DNA is cleaved and added to CRISPR array.
- Transcription of locus
- CRISPR RNA processing
- CRISPR RNA is cleaved into gRNAs by nuclease.
- The nuclease must be complexed with tracrRNA.
- RNA-guided targeting of viral element.
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Inactive Cas9 nuclease binds to gRNA and tracrRNA and becomes activated.
- Recognizes a complementary target sequence and cleaves it.
- RESULT: Recombination or Deletion.
Why is Cas9 inactive until it binds to gRNA and tracrRNA complex?
If it was activated it could spontaneously react to any DNA nearby.
Two types of nuclease-induced genome editing.
- Homology directed repair:
- Harder to do but fewer errors
- Non-homologous end joining
- Extremely error prone.
Describe the CRISPR/Cas system?
-
CRISPR array:
- Protospacers and short repeats
- Pre-crRNA is then joined with RNase 3, tracrRNA, and Cas9
- The complex cleaves the crRNAs
- The complex then looks for a target sequence (protospacer) which must be adjacent to a PAM (Protospacer adjacent motif).
- The complex then binds downstream (3’ ) of PAM sequence
- Cleaves both strands upstream of PAM
- Then the complex unbinds.
Are tracrRNA and gRNA comined into one in the Lab?
YEA
2 components needed for Lab based CRISPR/Cas9
Guide RNA (gRNA) - contains both tracrRNA and gRNA
Cas9 nuclease
Explain the PAM sequence
- Specific for each bacterial species
- Found directly downstream of the target.
- Required for Cas9 to work.
- Cas9 partially unwinds the the DNA.
- Thought to be present in every gene.
Requirements of CRISPR/Cas in a lab
- The sequence is unique compared to the rest of the genome.
- The target is present immediately upstream of a PAM
- PAM sequence is NGG.
What does homology directed repair require?
A template
Explain Cas9 nuclease
-
Two endonuclease activities are present in a complex.
- This means you can inhibit one and then selectively nick a single strand.
- Using two different Cas9 complexes each with one domain inhibited. You can make a large change to the genome by cutting only one strand a distance apart. Then using a template (homologous directed repair) to splice it in.
- This means you can inhibit one and then selectively nick a single strand.
Doubly inhibited Cas9 can be used for what?
To hold a transcriptional activator or repressor to activate or repress a target gene.
Hold GFP to ID a specific segment of the chromosome.
How can catalytically dead Cas9 be used?
- Neutered Cas9 can be used to activate or inactivate transcription of histones
- By binding a methylase to the complex DNA can be methylated using Cas9.
- Methylation decreases gene expression
- Demethylase can also be used.
- Demethyation increases gene expression.
- By binding a methylase to the complex DNA can be methylated using Cas9.
Limits of CRISPR/Cas in area of effect?
- Germline cells can be modded to effect whole animal.
- Somatic cells can be modded to effeect specific cells or tissues.
Application of CRISPR to treat cancer
- IF an activated protein is causing cancer you could code a stop codon before the protein, and add the DNA back into the patient.
- This would knock out the mutated protein.
Uses of CRISPR in the clinic
- Precision therapy
- Must ensure gRNA cant also bind elsewhere or there will be unintended side effects.
- Disease modeling
- Drug screening
